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人红细胞蛋白4.2:异构体表达、差异剪接及染色体定位

Human erythrocyte protein 4.2: isoform expression, differential splicing, and chromosomal assignment.

作者信息

Sung L A, Chien S, Fan Y S, Lin C C, Lambert K, Zhu L, Lam J S, Chang L S

机构信息

Department of AMES-Bioengineering, University of California, San Diego 92093-0643.

出版信息

Blood. 1992 May 15;79(10):2763-70.

PMID:1350227
Abstract

Human protein 4.2 (P4.2) is a major membrane skeletal protein in erythrocytes. Individuals with P4.2 deficiency exhibit spherocytosis and experience various degrees of hemolytic anemia, suggesting a role for this protein in maintaining stability and integrity of the membrane. Molecular cloning of P4.2 cDNAs showed that P4.2 is a transglutaminaselike molecule in erythrocytes but lacks the essential cysteine for cross-linking activity. Two cDNA isoforms have been identified from a human reticulocyte cDNA library, with the long isoform containing a 90-base pair (bp) in-frame insertion encoding an extra 30 amino acids near the N-terminus. Characterization of the P4.2 gene suggests differential splicing as the mechanism for generating these two cDNA isoforms. The donor site for the short isoform (P4.2S) agrees better with the consensus than the donor site for the long isoform (P4.2L) does. Expression of P4.2L was detected by a long-isoform-specific antibody raised against a peptide within the 30-amino acid insert. Western blot analyses showed P4.2L to be a minor membrane skeletal protein in human erythrocytes with an apparent molecular weight (mol wt) of approximately 3 Kd larger than the major protein 4.2, P4.2S. By in situ hybridization of a full-length 2.4-kilobase (kb) cDNA to human metaphase chromosomes, the gene for P4.2 was mapped to bands q15-q21 of chromosome 15, and it is not linked to the gene for coagulation factor XIIIa (plasma transglutaminase, TGase).

摘要

人蛋白4.2(P4.2)是红细胞中的一种主要膜骨架蛋白。P4.2缺乏的个体表现出球形红细胞增多症,并经历不同程度的溶血性贫血,这表明该蛋白在维持膜的稳定性和完整性方面发挥作用。P4.2 cDNA的分子克隆表明,P4.2是红细胞中的一种类转谷氨酰胺酶分子,但缺乏交联活性所必需的半胱氨酸。从人网织红细胞cDNA文库中鉴定出两种cDNA异构体,长异构体在N端附近含有一个90个碱基对(bp)的框内插入片段,编码额外的30个氨基酸。P4.2基因的特征表明,差异剪接是产生这两种cDNA异构体的机制。短异构体(P4.2S)的供体位点比长异构体(P4.2L)的供体位点更符合共有序列。通过针对30个氨基酸插入片段内的肽产生的长异构体特异性抗体检测到P4.2L的表达。蛋白质印迹分析表明,P4.2L是人类红细胞中的一种次要膜骨架蛋白,其表观分子量(mol wt)比主要蛋白4.2即P4.2S大约大3 Kd。通过将全长2.4千碱基(kb)的cDNA与人中期染色体进行原位杂交,将P4.2基因定位到15号染色体的q15-q21带,并且它与凝血因子XIIIa(血浆转谷氨酰胺酶,TGase)的基因不连锁。

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